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ABSTRACT
Puslane (Portulaca oleracea) has been identified for cultivation as a food crop
since its identification as an exceptionally rich source of bioprotective substances
(α-linolenic acid, linoleic acid, antioxidants, vitamins) which are considered
essential for growth, development and disease prevention. Also its short
vegetative period and almost all year round production makes it more favourable
or cultivation.
Many studies have been conducted to show the effect of different plant nutrition
on both crop production as well as the nutritional value of the plant. However little
is known about the suitable temperature and day length conditions necessary for
optimizing the nutritional value of the plants i.e. greater fatty acids concentrations
and lesser organic acids, and improving upon its agronomic potentials. The aim
of this study therefore was to determine the effects of temperature and day
length on the concentration of fatty acid and organic acid in leaves of purslane
and also its influence on crop production. Three microspecies P. sativa, P. nitida,
P. papillatostellulata from the Portulaca complex were used in this study. Plants
were grown under four different day/night temperature conditions (34/28, 28/22,
22/16, 16/100C), long day (LD) and short day (SD) for 8 weeks. We determined
plant height, leaf length, plant number of internodes, leaf and stem fresh weights
and dry weights, moisture content, percentage leaf dry weight in plant fresh
weight during the experiment. Plant leaves were also harvested at 8-true leaf
stage for fatty acid analysis as well as the organic acid concentrations. We found
that plant height, leaf length, number of plant internodes, average length of
internodes, leaf and stem fresh and dry weight, net plant fresh and dry weights of
all microspecies decreased as the temperature decreased from 34-160C in both
day length regimes. The commercial green-leaf P. sativa recorded the highest
measurements for all the parameters mentioned above (LD, SD) with the
exception of the leave dry weight and percentage moisture content. With these
measurements, P. nitida was similar to P. sativa especially within the 34-220C
temperature condition, LD and SD. Percentage leaf dry weight in whole plant
fresh weight was also significantly increased in P. nitida at temperatures 34-220C,
LD and SD. All plants except P. nitida significantly increased in oxalic acid
concentrations as the temperature decreased to 16/100C in both day length
regimes. Significant decreasing trends in ascorbic acid and the major fatty acids
determined (α-linolenic acid, linoleic acid and palmitic acid) were also found as
the temperature condition reduced to 16/100C especially with the P. nitida
microspecies. There was however no significant differences in the major fatty
acids determined among the three microspecies in the 34-220C temperature
condition, long day and short day. Our results therefore conclude that decreasing
the temperature for growth to as low as 16/100C reduced plant growth and
performance (even death) and decreased the nutritional value of all plants
microspecies. Our results also indicate potential agronomic traits of local
microspecies P. nitida.
The present study was also undertaken to explore the ameliorative effect of
purslane on a mice model of human acute ulcerative colitis (UC). Acute colitis
was induced by exposing female C57BL/6 mice to 3.5% DSS in drinking water
for 8 days.
Five groups of mice were used: three of them received in their chow 24% (6 g)
powdered purslane leaves which contained (4800 mg ALA), 8% (2 g) leaves
which contained (1600 mg ALA) and 0.8% (0.2 g) leaves which contained (160
mg ALA).
The combined chow and leaves were given ad libitum for 10 days prior to DSS
administration and this continued till the end of the experiment. DSS was also
induced in one control group fed with standard diet. At the end of the experiment,
mice were sacrificed and colonic damage was assessed both histologically and
biochemically. Plasma fatty acids, colonic length, disease activity index (DAI) and
MPO were determined. Administration of purslane leaves induced a significant
increase in plasma DHA and in the 24% treated group and not 8% or 0.8%
groups as opposed the normal control. EPA was not found in any of the groups.
Administration of DSS resulted in a significant development of ulceration in the
colon along with a rise disease activity and MPO. Dry powdered puslane leaves
provided in the food at different concentrations did not significantly attenuate
DSS-induced colonic inflammation along with MPO and DAI. Mild protectiveness
was however seen among the 24% and 8% fed groups histologically. The reason
behind the mild protectiveness observed histologically and not biochemically is
unclear. The inability of purslane leaves to mitigate ulceration caused by DSS
might have been related to the ingestion of other organic compounds (organic
acids, coumarins, alkaloids, anthraquinones) in the leaves which have been
suggested to have toxic effects in higher concentrations, low concentrations of
ALA used or the non-conversion of ALA to EPA. It is concluded that purslane
may be a novel food factor for preventing experimental UC if the omega 3 active
components are isolated from the leaves and purified devoid of other organic
compounds. Further research in this plant is needed to identify its therapeutic
effects on UC.